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利用表面展示的几丁质结合结构域将乳链菌肽产生菌 Lactococcus lactis 固定在几丁质上。

Immobilization of nisin producer Lactococcus lactis strains to chitin with surface-displayed chitin-binding domain.

机构信息

Department of Food Engineering, Faculty of Engineering, University of Pamukkale, Denizli, Turkey.

出版信息

Appl Microbiol Biotechnol. 2013 May;97(10):4577-87. doi: 10.1007/s00253-013-4700-9. Epub 2013 Jan 26.

Abstract

In this study, nisin producer Lactococcus lactis strains displaying cell surface chitin-binding domain (ChBD) and capable of immobilizing to chitin flakes were constructed. To obtain ChBD-based cell immobilization, Usp45 signal sequence with ChBD of chitinase A1 enzyme from Bacillus circulans was fused with different lengths of PrtP (153, 344, and 800 aa) or AcmA (242 aa) anchors derived from L. lactis. According to the whole cell ELISA analysis, ChBD was successfully expressed on the surface of L. lactis cells. Scanning electron microscope observations supported the conclusion of the binding analysis that L. lactis cells expressing the ChBD with long PrtP anchor (800 aa) did bind to chitin surfaces more efficiently than cells with the other ChBD anchors. The attained binding affinity of nisin producers for chitin flakes retained them in the fermentation during medium changes and enabled storage for sequential productions. Initial nisin production was stably maintained with many cycles. These results demonstrate that an efficient immobilization of L. lactis cells to chitin is possible for industrial scale repeated cycle or continuous nisin fermentation.

摘要

在这项研究中,构建了能够固定在几丁质薄片上的展示细胞表面几丁质结合域(ChBD)的乳球菌乳亚种纳豆菌生产菌株。为了进行基于 ChBD 的细胞固定化,将来自解淀粉芽孢杆菌的几丁质酶 A1 酶的 Usp45 信号序列与不同长度的 PrtP(153、344 和 800 aa)或 AcmA(242 aa)锚定物融合。根据全细胞 ELISA 分析,ChBD 成功表达在乳球菌细胞表面。扫描电子显微镜观察结果支持结合分析的结论,即表达带有长 PrtP 锚(800 aa)的 ChBD 的乳球菌细胞比具有其他 ChBD 锚的细胞更有效地结合几丁质表面。获得的纳豆菌生产者对几丁质薄片的结合亲和力在培养基变化过程中将它们保留在发酵中,并能够进行连续生产的储存。初始纳豆菌素的生产稳定保持了多个循环。这些结果表明,乳球菌细胞与几丁质的有效固定化可能用于工业规模的重复循环或连续纳豆菌素发酵。

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